Volume 82, Issue 1, Pages (April 2014)

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Volume 82, Issue 1, Pages 109-124 (April 2014) Calcineurin Signaling Regulates Neural Induction through Antagonizing the BMP Pathway  Ahryon Cho, Yitai Tang, Jonathan Davila, Suhua Deng, Lei Chen, Erik Miller, Marius Wernig, Isabella A. Graef  Neuron  Volume 82, Issue 1, Pages 109-124 (April 2014) DOI: 10.1016/j.neuron.2014.02.015 Copyright © 2014 Elsevier Inc. Terms and Conditions

Figure 1 Anterior Defects in CnB1 Mutant and CsA-Treated Embryos (A) Scanning electron micrographs of E9.5 embryos; forebrain (arrow). (B) Pax6 immunostaining of E9.0 sagittal sections. (C–F) qRT-PCR analysis of germ layer markers in e7.5 CnB1 control and mutant embryos. (C) Fezf1 (p = 0.0028); Fezf2 (p = 0.0011); Six3 (p = 0.0103). (D) Gata6 (p = 0.0768). (E) Brachyury (T) (p < 0.0001). (F) Krt8 (p = 0.0295). (G) Cartoon of in utero CsA treatment. The red region indicates the critical period during which CaN activity is required in the developing embryo. (H–K) qRT-PCR analysis of germ layer markers in E7.5 control and CsA-treated embryos. (H) Fezf1 (p = 0.0230); Fezf2 (p = 0.0086); Six3 (p = 0.0001). (I) Gata6 (p = 0.2673). (J) Brachyury (T) (p = 0.0010). (K) Krt8 (p = 0.7345). (L) Pax6 immunostaining of E9.0 control and CsA-treated embryos. Data are shown as mean ± SEM. Scale bar in (B) and (L) represents 100 μm. See also Figure S1. Neuron 2014 82, 109-124DOI: (10.1016/j.neuron.2014.02.015) Copyright © 2014 Elsevier Inc. Terms and Conditions

Figure 2 Calcineurin Activity Is Required for Neural Differentiation of Murine and Human ESCs (A) Schematic representation of in vitro ESC to neural differentiation using Sox1-GFP reporter murine ESCs. (B) Quantification of Sox1-driven GFP (=Sox1-GFP) expression on d12 by FACS analysis. % of GFP-positive cells: NT, 27.5%; d3–d12 FK506- and CsA-treated (FK/CsA), 3.84%. (C) Sox1-GFP expression of NT and FK/CsA-treated (d3–d12) cells on d12. (D) Critical time window during which calcineurin (CaN) activity is necessary for neural induction. Cells were treated with FK/CsA during the indicated time windows (gray bars) of in vitro murine ESC differentiation. On d12, GFP expression of each group was measured by FACS analysis and/or western blot to quantify neural induction. (E) Quantification of Sox1-GFP expression on d12 by FACS analysis (mean ± SEM). Cells were treated with indicated molecules during d3–d12 or d3–d8. FACS data were normalized to the NT control group. p value compared to NT: FK/CsA d3–d12 (n = 5), p < 0.0001; FK/CsA d3–d8 (n = 5), p < 0.0001; FK506 d3–d8 (n = 3), p = 0.0097; CsA d3–d8 (n = 3), p = 0.0028. (F) Confocal immunofluorescence images of NT and FK/CsA-treated (d3–d8) cells on d15 using antibodies against GFP and pan-neuronal marker β-III-tubulin. Scale bar represents 10 μm. (G) Immunofluorescence images of NT and FK/CsA-treated H1 cells on d11 of hESC differentiation using antibodies against SOX2 and PLZF. Scale bar represents 50 μm. (H and I) Microarray gene expression profiles of indicated genes on d4, d6, d8, and d12 cells of in vitro murine ESC differentiation. CaN was inhibited with FK/CsA from d3 to d8. (H) Neuroectoderm markers. (I) Pluripotency, endoderm, mesoderm, and ectoderm markers. Samples were collected from three independent experiments of in vitro differentiation. Data are shown as mean ± SEM. See also Figure S2. Neuron 2014 82, 109-124DOI: (10.1016/j.neuron.2014.02.015) Copyright © 2014 Elsevier Inc. Terms and Conditions

Figure 3 FGF8-Regulated Ca2+ Entry Enhances Neural Induction (A) Quantification of Sox1-GFP expression by FACS. % of GFP positive cells: NT, 32.3%; FGF8, 50.5%; FGF17, 49.5%. (B) Immunoblot analysis of Sox1-GFP and Sox1 after treatment with FGF8a, FGF8b, or FK/CsA. Brg1 and Hsp90 are loading controls. (C) Quantification of Sox1-GFP expression by FACS. % of Sox-1 GFP positive cells: NT, 32.3%; FGF2, 21.9%; FGF4, 30%. (D) Immunoblot analysis of Sox1-GFP and Sox1 after treatment with FGF2 and FGF4. (E) SOX2 and PLZF immunostaining of hESC treated with the indicated molecules and harvested on d11 of differentiation. Scale bar represents 50 μm. (F) Quantification of Sox1-GFP expression by FACS analysis (mean ± SEM). FACS data were normalized to the NT control group. (G) Immunoblot analysis of GFP and Sox1 expression after treatment with the indicated molecules. In (A)–(D), (F) and (G), cells were treated with the indicated growth factors or small molecules during d3–d8 of in vitro murine ESC differentiation and harvested on d12 for analysis. See also Figure S3. Neuron 2014 82, 109-124DOI: (10.1016/j.neuron.2014.02.015) Copyright © 2014 Elsevier Inc. Terms and Conditions

Figure 4 CaN Antagonizes BMP Signaling during Neural Differentiation of ESCs (A–C) Murine ESCs were treated with the indicated molecules from d3 to d8 of in vitro differentiation. (A) Microarray gene expression profiles of BMP-regulated genes on d4, d6, d8, and d12. Graphs are shown as mean ± SEM. (B) Quantification of Sox1-GFP- and Flk1-positive cells on d12 by FACS analysis. (C) Quantification of Sox1-GFP-positive cells on d12 by FACS analysis. % of GFP-positive cells: NT, 27.5%; FK/CsA, 4.68%; Noggin, 74%; Noggin+FK/CsA, 54.2%; BMP4, 0.951%. (D) Immunoblot analysis shows the level of pSmad1/5C-term, Smad1, and Smad5 in d6 EBs treated with the indicated molecules for 1 hr. (E) Immunoblot analysis of nuclear and cytoplasmic fractions (d5 EBs) for pSmad1/5C-term, pSmad1linker, Smad1/5, CnB1, TATA-binding protein (TBP) (nuclear loading control), and β-tubulin (cytoplasmic loading control). Cells were treated with the indicated molecules for 1 hr. OA, okadaic acid. (F) Immunoblot analysis of HaCaT whole-cell extracts for pSmad1/5 C-term, Smad1, and actin. BMP2 and FK/CsA treatment: 15 min. (G) The effect of constitutively active CaN on pSmad1/5 C-term in d2 human EBs differentiated from hESCs expressing control and constitutively active CaN, respectively. Immunoblot analysis shows the level of pSMAD1/5C-term, SMAD1/5, CnB1, NFATc4, CnA, GFP (expression control), and HSP90 (loading control). (H) In vitro phosphatase assay using nuclear and cytoplasmic extracts from BMP4-stimulated d8 EBs. Immunoblot analysis detects the levels of pSmad1/5C-term, Smad1/5, TBP, and tubulin after the assay. CIP, calf intestinal alkaline phosphatase. See Experimental Procedures for details. See also Table S1 and Figure S4. Neuron 2014 82, 109-124DOI: (10.1016/j.neuron.2014.02.015) Copyright © 2014 Elsevier Inc. Terms and Conditions

Figure 5 Smad1/5 Proteins Are the Critical Targets of CaN during Neural Induction (A and B) in vitro differentiation of a murine ESC line harboring ERT2CreERT2; NFATc1L/L c2−/− c3L/Lc4 −/− in which the floxed alleles of NFATc1 and NFATc3 were removed by 4-OHT-regulated nuclear import of ERT2CreERT2. 4-OHT was added at the ESC stage and FK/CsA from d3 to d8. (A) Immunoblot analysis of d8 EBs using antibodies against NFATc3, pSmad1/5C-term, Smad1/5, and actin (loading control). pNFATc3: phosphorylated (arrow), NFATc3: dephosphorylated (arrowhead); ∗ indicates a nonspecific band. (B) Immunoblot analysis of d12 EBs using antibodies against NFATc3, Sox1, and Hsp90 (loading control). (C) FACS analysis of Sox1-GFP expression was used to quantify the percentage of neural induction following inhibition of BMP signaling in the presence or absence of CaN activity or FGF signaling. Cells were treated with indicated molecules during d3–d8. FACS data were normalized to the NT control group. (D) Inhibition of CaN has no effect on SOX2 and PLZF expression of hESCs in the presence of dual SMAD inhibition with a combination of SB431542, an ALK inhibitor, and LDN193189, a BMP inhibitor. Scale bar represents 50 μm. (E) Immunoblot analysis for pSmad1/5C-term, Smad1/5, and actin (loading control) in d4 murine EBs treated with the indicated molecules. Ionomycin, FK/CsA, and FGF8: 1 hr; FGFR-Fc and Pyr3: 3 hr. See also Figures S5 and S6. Neuron 2014 82, 109-124DOI: (10.1016/j.neuron.2014.02.015) Copyright © 2014 Elsevier Inc. Terms and Conditions

Figure 6 Increased BMP Signaling in CnB1 Mutant and CsA-Treated Embryos (A and B) qRT-PCR analysis of BMP-regulated genes at E7.5 (A) CnB1 control and mutant embryos. Mixl1 (p = 0.0053); Smad6 (p = 0.0030); Mesp1 (p = 0.0214); Eomes (p = 0.0108). (B) Control and CsA-treated embryos; pregnant females were injected with CsA on E6.25 and E6.75. Mixl1 (p = 0.0002); Smad6 (p = 0.0073); Mesp1 (p = 0.0006); Eomes (p = 0.0002). Data are shown as mean ± SEM. (C and D) Immunoblot of NFATc3, pSmad1/5C-term, Smad1, Smad5, and actin in (C) E7.5 control and CsA-treated embryos; (D) E8.0 CnB1 control and mutant headfolds. pNFATc3: phosphorylated (arrow); NFATc3: dephosphorylated (arrowhead); ∗ indicates a nonspecific band. Neuron 2014 82, 109-124DOI: (10.1016/j.neuron.2014.02.015) Copyright © 2014 Elsevier Inc. Terms and Conditions

Figure 7 Modulation of BMP Signaling by FGF/Ca2+/CaN Signaling Model depicting the proposed mechanism for inhibition of BMP signaling by CaN. FGF signaling triggers an increase of intracellular Ca2+, which activates the CaN phosphatase complex consisting of CnA, CnB, and CaM. Activated CaN specifically dephosphorylates pSmad1/5C-term, thereby opposing BMP signaling. A lack of CaN activity results in an increase of nuclear pSmad1/5C-term and an enhanced or ectopic activation of BMP-regulated transcription. BMPR, BMP receptor; CnA, calcineurin subunit A; CnB, calcineurin subunit B; FGFR, FGF receptor; TRPC, canonical transient receptor potential. Neuron 2014 82, 109-124DOI: (10.1016/j.neuron.2014.02.015) Copyright © 2014 Elsevier Inc. Terms and Conditions